Comparative SAXS and DSC study on stratum corneum structural organization in an epidermal cell culture model (ROC): impact of cultivation time.

Cell cultured skin equivalents present an alternative for dermatological in vitro evaluations of drugs and excipients as they provide the advantage of availability, lower variability and higher assay robustness compared to native skin. For penetration/permeation studies, an adequate stratum corneum barrier similar to that of human stratum corneum is, however, a prerequisite. In this study, the stratum corneum lipid organization in an epidermal cell culture model based on rat epidermal keratinocytes (REK organotypic culture, ROC) was investigated by small-angle X-ray scattering (SAXS) in dependence on ROC cultivation time and in comparison to native human and rat stratum cornea. In addition, the thermal phase behavior was studied by differential scanning calorimetry (DSC) and barrier properties were checked by measurements of the permeability of tritiated water. The development of the barrier of ROC SC obtained at different cultivation times (7, 14 and 21 days at the air-liquid interface) was connected with an increase in structural order of the SC lipids in SAXS measurements: Already cultivation for 14 days at the air-liquid interface resulted overall in a competent SC permeability barrier and SC lipid organization. Cultivation for 21 days resulted in further minor changes in the structural organization of ROC SC. The SAXS patterns of ROC SC had overall large similarities with that of human SC and point to the presence of a long periodicity phase with a repeat distance of about 122Å, e.g. slightly smaller than that determined for human SC in the present study (127Å). Moreover, SAXS results also indicate the presence of covalently bound ceramides, which are crucial for a proper SC barrier, although the corresponding thermal transitions were not clearly detectable by DSC. Due to the competent SC barrier properties and high structural and organizational similarity to that of native human SC, ROC presents a promising alternative for in vitro studies, particularly as it can be obtained under overall rather straightforward cell culture conditions and thus low assay costs.

Preservation of liquid drug preparations for oral administration.

The aim of this study was to investigate functional interactions between sorbic acid, alcoholic cosolvents, and pH with respect to pharmacopeial requirements for the antimicrobial preservation of oral liquids. Twenty-seven test formulations of sugar-free syrups with varying amounts of glycerol (18-36%), propylene glycol (4-21%), and sorbic acid (0-0.15%) and with different pH values (5-8) were tested for antimicrobial preservation efficacy after inoculation with spores of Aspergillus niger. Multivariate data analysis revealed that at pH 5 the minimum concentration of sorbic acid necessary for a tenfold decrease of viable spores ranges between 0.08% and 0.10% exhibiting only minor dependence on the cosolvents concentration. Various interactions between sorbic acid and cosolvents could be observed and were discussed on basis of the degree of dissociation and distribution of sorbic acid. All tested preparations, even those free of sorbic acid, met the criteria for oral products with aqueous bases according to USP32-NF27 and JP XV which claim no increase from the initial spore count at 14 and 28 days. The EP requirement, not less than 1 log(10) reduction from the initial count at 14 days, was only met by preparations with pH 5 and not less than 0.15% sorbic acid.